Overexpression of OsSWEET5 in Rice Causes GrowthRetardation and Precocious SenescenceYong Zhou1, Li Liu2, Weifeng Huang1, Meng Yuan1, Fei Zhou1, Xianghua Li1, Yongjun Lin1*
1 National Key Laboratory of Crop Genetic Improvement and National Centre of Plant Gene Research, Huazhong Agricultural University, Wuhan, China, 2 Plant
Reproductive Biology, University of California Davis, Davis, California, United States of America
Abstract
As a novel sugar transporter family, SWEETs play important roles in plant growth and development. Here, we characterizeda SWEET gene named OsSWEET5 through its overexpression in rice. Heterologous expression assay indicated that OsSWEET5encoded a galactose transporter in yeast. OsSWEET5-overexpressing plants displayed the phenotypes of growth retardationand precocious senescence at seedling stage. GC-MS analysis showed that the sugar levels were largely altered in the leavesof the OsSWEET5-overexpressing plants. Molecular analysis revealed that these phenotypes might be due to thetranscriptional changes of the genes involved in sugar metabolism and transport. In addition, the transgenic plants showeda lower level of auxin with altered transcription of genes involved in auxin signaling and translocation pathways. However,no obvious phenotype was observed between the amiRNA-OsSWEET5 transgenic lines and WT plants, which could be aresult of the functional redundancy of the galactose transporters in rice. Taken together, our findings suggest thatOsSWEET5 plays a crucial role in regulating the crosstalk between sugar and auxin in rice.
Citation: Zhou Y, Liu L, Huang W, Yuan M, Zhou F, et al. (2014) Overexpression of OsSWEET5 in Rice Causes Growth Retardation and Precocious Senescence. PLoSONE 9(4): e94210. doi:10.1371/journal.pone.0094210
Editor: Jinfa Zhang, New Mexico State University, United States of America
Received August 13, 2013; Accepted March 13, 2014; Published April 7, 2014
Copyright: � 2014 Zhou et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permitsunrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: This research was funded by the National High Technology Research and Development Program of China (863 Program), the National Natural ScienceFoundation of China and the National Program of Transgenic Variety Development of China. The funders had no role in study design, data collection and analysis,decision to publish, or preparation of the manuscript.
Competing Interests: The authors have declared that no competing interests exist.
* E-mail: [email protected]
Introduction
Plants absorb solar energy during photosynthesis for fixation of
carbon in leaves and produce photoassimilates, which are
transported into storage pools such as plastidic starch or vacuolar
sugars. The transportation and distribution of photoassimilates in
higher plants from phototrophic to heterotrophic cells and tissues
depend on the activities of numerous transporters [1]. Carbohy-
drates are transported from the source to photosynthetically
inactive sink tissues mainly in the form of sugar, especially sucrose.
Cell-to-cell transport of sucrose depends on the activities of
plasma-membrane-located sucrose transporters (SUTs) [2]. And
sucrose can be hydrolysed by cell-wall-bound invertases to glucose
and fructose, which can be transported into cells via monosac-
charide transporters (MSTs) [3]. Normal transportation of sugars
from source leaves to sink tissues or organs is very important for
plant growth and development [4]. Imbalanced carbohydrate
distribution between source and sink at the whole plant level can
cause decreased expression of photosynthetic genes, and reduce
the growth rate of the plant [5]. For example, ZmSUT1 functions
in phloem load sucrose in maize leaves, and the mutants of
ZmSUT1 hyperaccumulated soluble sugars in leaves, displaying the
phenotypes of leaf chlorosis and reduced growth [6,7]. OsSUT2 is
involved in sucrose transport across the tonoplast from the vacuole
lumen to the cytosol in rice, and ossut2 showed obviously increased
levels of sucrose, glucose and fructose compared with the controls,
leading to a phenotype of growth retardation [8]. AtSWEET17 is
the first vacuolar fructose transporter, which can export fructose
out of the vacuole; and AtSWEET17 mutations caused stunted
growth and affected seed yield, suggesting that AtSWEET17 can
control the fructose level of leaf in Arabidopsis [9]. However, the
mechanism of the source-sink interaction for sugar transport
remains elusive.
Many studies have demonstrated a potential link between sugar
and auxin signaling pathways [10,11,12,13]. On one hand, auxin
can regulate sugar synthesis and transport in plants. For example,
OsSAUR39 acts as a negative regulator of auxin synthesis and
transport in rice, and overexpression of OsSAUR39 in rice causedsugar accumulation and transcriptional changes of the genes
involved in sugar synthesis and transport [14,15]. In tomato, a
member of auxin response factor (ARF) gene family named SlARF4plays a major role in mediating the auxin control of sugar
metabolism during fruit development [16]. On the other hand, as
signaling molecules, sugars play central roles in regulating the
expression of auxin-responsive genes to modulate auxin biosyn-
thesis and signaling. For example, sugar levels can regulate the
transcript of ZmYUC to modulate the tryptophan-dependent auxinbiosynthesis in developing maize kernels [12]. A previous study
also has showed that IAA biosynthesis is regulated by endogenous
sugar levels [17]. And it has been reported that the control of
glucose to root growth and development in Arabidopsis is
probably through auxin signaling [13]. In addition, some studies
have suggested that auxin-induced growth can be inhibited by
galactose [18,19,20], and this inhibition may be due to the
inhibition of auxin-induced H+-excretion needed for the initiation
of rapid elongation or the inhibition of cell wall synthesis [21].
There are a number of sugar transporters which are involved in
galactose transport and play important roles in many physiological
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pathways in plants. CkHUP2 (Chlorella kessler hexose uptake 2) is a
high-affinity transporter for galactose in Chlorella kessleri, which may
function in the import of organic compounds during the
heterotrophic growth of plant cells [22]. OsMST4, a functional
monosaccharide transporter capable of transporting galactose, is
expressed in both the source and sink tissues, and is suggested to
participate in many developmental stages in rice [23]. In
Arabidopsis, the sugar transport protein AtSTP1, a high-affinity
H+-monosaccharide symporter which can transport galactose,
plays important roles in the uptake of extracellular sugars by the
embryo and in seedlings [24,25]. A subsequent research found that
AtSTP1 is expressed in guard cells and has a role in the import of
monosaccharide into guard cells during night [26]. AtSTP11,
which is exclusively expressed in pollen tubes, is another high
affinity hexose-specific H+-symporter involved in galactose trans-
port, and plays a role in the supply of monosaccharides to growing
pollen tubes [27]. AtSTP14 is the first plant transporter specific for
galactose and is suggested to be involved in the retrieval of cell
wall-derived galactose; meanwhile its expression is regulated by
darkness, sugar starvation, senescence and drought stress, which
eventually induce cell wall degradation [28]. AtSTP2 also could
serve in the uptake of galactose into the developing male
gametophyte, and galactose is proposed to be a degradation
product from cell-wall components [29]. Therefore, it can be
speculated that galactose transporters probably participate in cell
wall galactose recycling or/and galactose supplying to tissues or
organs during different developmental stages in plants.
The MtN3/saliva proteins were first described in Medicago
truncatula [30]. Recent studies have shown that many members of
MtN3/saliva family belong to the SWEET subfamily and can
mediate sugar transport, and the sugar transporters probably
supply carbohydrates to various tissues in both monocots and
dicots [31,32]. For example, OsSWEET11 and OsSWEET14 not
only mediate the glucose import and efflux in human embryonic
kidney (HEK) 293T cells and Xenopus oocytes, but also serve as
low-affinity sucrose transporters [31,33]. OsSWEET11 showed
high expression levels in panicles and anthers, and OsSWEET11-
RNAi transgenic plants showed a severely reduced fertility and
even complete sterility, suggesting that OsSWEET11 plays an
important role in regulating the reproductive development of rice
[32,34]. OsSWEET14 homozygous T-DNA insertion mutant
plants showed remarkable delayed growth compared with the
heterozygous mutant plants [35]. In Arabidopsis, AtSWEET11 and
AtSWEET12 function as low-affinity transporters for the efflux of
sucrose from phloem parenchyma cells into the apoplast, and
single AtSWEET11 or AtSWEET12 mutants showed no visible
phenotype, but the atsweet11atsweet12 double mutant plants
displayed the phenotype of reduced growth [33]. AtSWEET17
acts to export fructose out of the vacuole and has a role in
carbohydrate partitioning in plants, which can regulate the
developmental processes of plants [9]. AtSWEET16 can catalyze
the transport of glucose, fructose, and sucrose, and AtSWEET16-
overexpressing plants displayed significant alterations in sugar
levels as well as in different development processes like germina-
tion, growth, and stress tolerance [36]. Therefore, SWEETs may
be key regulators in plant growth and development.
In this paper, we characterized a member of SWEETs named
OsSWEET5 in rice, which encoded a sugar transporter protein
involved in galactose transport. The OsSWEET5-overexpressing
plants showed retarded growth in the early seedling stage with
altered sugar metabolism and transport as well as inhibited auxin
signaling and translocation. The study was aimed to achieve a
better understanding on the possible physiological functions of
OsSWEET5 and thus to optimize the transport and reserve of
carbohydrates to raise the yield of rice.
Materials and Methods
Plant materials and growth conditionsZhonghua 11 (Oryza Sativa L. ssp. Japonica cv. Zhonghua 11) was
used in this study. OsSWEET5 transgenic plants and Zhonghua 11(as the wild type) were planted in the field of Huazhong
Agricultural University (Wuhan, China).
Plasmid construction and rice transformationFor POsSWEET5::GUS vector construction, OsSWEET5 promoter
(about 2.3 kb 59-upstream fragment of OsSWEET5) was amplifiedusing rice genomic DNA as a template. The DNA fragment was
inserted into the pDX2181 vector [37]. For overexpression vector
construction, the DNA fragment was amplified, digested with KpnI and Xba I and ligated to the pCAMBIA1300 under the control ofthe 35S promoter. Constructs were transformed into Zhonghua 11
as previously described [38]. The independent OsSWEET5-overexpressing transgenic plants were further confirmed by PCR
assay and Southern blot [38]. The method of Southern blot was
also described in Methods S1. The PCR program was as follows:
94uC for 5 min, followed by 30 cycles of 94uC for 1 min, 58uC for1 min, and 72uC for 1 min, 72uC for 7 min. The sequences ofprimers are listed in Table S1.
Histochemical assayThe histochemical GUS assay was performed as previously
described [37]. Samples from independent POsSWEET5::GUStransgenic plants were incubated at 37uC in GUS reagent forabout 10 h after 15 min vacuum filtration. All the samples were
destained by 75% (v/v) alcohol and observed subsequently using a
dissecting microscope (Leica, Germany).
Subcellular localizationThe ORF of OsSWEET5 with the exception of stop codon was
amplified using the full-length cDNA clone J023023E05 (http://
cdna01.dna.affrc.go.jp/cDNA) as a template and cloned into the
pM999-35S-EGFP vector. Rice protoplasts transformation was
performed as described earlier [39]. GFP fluorescent signals were
observed and photographed using CLSM (Leica, Germany) after
20 h of dark culture at 28uC.
Functional characterization of OsSWEET5 in yeastYeast plasmids were kindly provided by Dr. Eckhard Boles,
Johann Wolfgang Goethe-Universität Frankfurt, Germany and the
vector backbones p426 and p413 were constructed as previously
described [40]. The HXT7 (hexose transporter 7) promoter wasamplified by using vector p426-pHXT7-HXT7 as template and
cloned into vector p413GPD to form p413-pHXT7 as negative
control. The HXT7 gene was amplified by using vector p426-pHXT7-HXT7 as template and inserted into p413-pHXT7 to
form p413-pHXT7-HXT7 as positive control. The ORF of
OsSWEET5 was amplified and cloned into p413-pHXT7, yieldingconstruct p413-pHXT7-OsSWEET5. These constructs were
transformed into a hexose transport-deficient yeast strain
EBY.VW4000 (MATa Dhxt1-17 Dgal2 Dstl1 Dagt1 Dmph2 Dmph3leu2-3,112 ura3-52 trp1-289 his3-D1 MAL2-8c SUC2) [41] andgrown on synthetic deficient medium containing either 2%
maltose (as control) or 2% glucose, 2% fructose, 2% mannose,
2% galactose, 2% sucrose, respectively. Due to the lack of all the
HXT genes, EBY.VW4000 no longer grows on monosaccharidesbut can grow on maltose. Synthetic medium consisted of 6.7 g/l
OsSWEET5 Regulates Growth and Senescence in Rice
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http://cdna01.dna.affrc.go.jp/cDNAhttp://cdna01.dna.affrc.go.jp/cDNA
Difco yeast nitrogen base (YNB) supplemented with essential
amino acids. The transformants were then grown overnight in
liquid minimum medium to OD600 = 1.0. A 4 ml aliquot of thetransformants and each of the three consecutive 1/10 dilutions
(0.1, 0.01, and 0.001) were spotted and incubated for 3–5 days at
30uC.
RNA extraction, RT-PCR, qRT-PCR and Northern blotanalysis
Total RNA was isolated using TRIzol reagent (Invitrogen,
Carisbad, CA, USA) according to the manufacturer’s instruction.
First-strand cDNAs were synthesized from RNase-free DNase I-
treated (Invitrogen, USA) total RNA to eliminate genomic DNA
contamination according to the manufacturer’s instruction. The
RT-PCR program was as follows: 94uC 3 min, followed by 28–30cycles of 94uC for 1 min, 58uC for 1 min, and 72uC for 30 s, andthen a final extension at 72uC for 7 min. Rice Actin1 was used asan internal control. qRT-PCR was performed with Applied
Biosystems 7500 Real-Time PCR System (Applied Biosystems,
Carlsbad, CA, USA) using SYBR Green I (TaKaRa, Japan) as
previously described [42]. Three replicates were performed for the
analysis of each gene. Rice Actin1 as an internal control and the
relative expression levels of target genes were determined as
described previously [43]. The sequences of the primers are listed
in Table S1. For Northern blot analysis, 15 mg of total RNA wasseparated in 1.2% (w/v) agarose gel, transferred to Hybond-N
nylon membrane (Amersham, USA), and hybridized with a PCR
fragment labeled with [a-32P] dCTP using a Random PrimerDNA Labeling Kit (TaKaRa, Japan). The hybridization signals
were obtained by autoradiography in Fujifilm FLA-5100 (Fujifilm,
Japan) according to the protocol described previously [44]. The
probe for Northern blot was amplified using PCR with primers
listed in Table S1.
Measurement of chlorophyll, auxin and sugar contentChlorophyll content measurement was carried out according to
a previous study [45]. Auxin was extracted and quantificated as
described previously [46]. For measurement of sugars, leaves from
OX2 and WT were first ground using PBS buffer (pH 7.0) after
being weighed. After centrifugation and resuspension in PBS
buffer (pH 7.0), samples mixed with internal standard (inositol,
Sigma, USA) were dried with dry N2 gas and derivatized using
N,O-bis[trimethylsilyl]-trifluoroacetamide (Alpha, USA): di-
methylformamide (Sigma, USA) (BSTFA: DMF, 1:1, v/v).
Afterwards, the derivatized sample extracts were diluted with
acetone and analyzed by GC-MS (SHIMADZU GCMS-QP2010
Plus) with HP-5 MS column (60 m60.32 mm60.25 mm) using themethods described previously [47,48] with modifications. The
quantification of sugars was performed with internal standard
method, and the retention times were as follows: galactose,
13.7 min and 14.75 min; sucrose, 27.466 min; glucose, 14.43 min
and 16.684 min; fructose, 12.355 min, 12.545 min and
12.629 min; and inositol, 19 min.
Results
Sequence analysis of OsSWEET5 in riceOsSWEET5 (TIGR ID: LOC_Os05g51090) consisting of four
exons and three introns and encoding a protein with 237 amino
acids was cloned from rice (cv Zhonghua 11) with an ORF of
714 bp. Phylogenetic analysis showed that OsSWEET5 was a
member of SWEETs Clade II subfamily [31]. The predicted
OsSWEET5 protein contained two MtN3/saliva domains in the
N- and C-terminal regions, which was in accordance with the
characteristics of the MtN3/saliva family (Figure S1).
Expression pattern of OsSWEET5qRT-PCR analysis revealed that OsSWEET5 was mainly
expressed in the floral organs at the heading stage, and was also
detectable in stem, root and senescing leaves (Figure S2). To
further examine the spatiotemporal expression pattern of OsS-
WEET5, we generated transgenic rice plants with the POsSWEET5::-
GUS construct and checked the GUS activity in five independent
transgenic plants. The results showed that GUS expression was
detected in the senescing leaves, stamen, pistil, hull, stem and root
(Figure 1).
Subcellular localization of OsSWEET5Most of SWEETs are small proteins which are predicted to have
seven transmembrane helices, with the first and last 3-transmem-
brane-helix-domain polypeptide fused via the middle transmem-
brane helix to form a 3+1+3 configuration structure [31,32]. In thepresent study, bioinformatic analyses using TMHMM (http://
www.cbs.dtu.dk/services/TMHMM/) and SOSUI (http://bp.
nuap.nagoya-u.ac.jp/sosui/) predicted that OsSWEET5 con-
tained seven transmembrane helices (Table S2, Figure S3)
[49,50]. The subcellular localization of OsSWEET5 was then
analyzed by transient expression of an OsSWEET5-GFP fusion
protein in rice protoplast. Confocal scanning laser microscopy
showed that GFP signals were observable at the plasma membrane
in OsSWEET5-GFP fusion vector (Figure 2A–D); whereas the
GFP control vector displayed fluorescence in the cytosol and
nuclei in the cells (Figure 2E–G), which suggested that OsSWEET5
encoded a plasma membrane protein.
Sugar transport ability of OsSWEET5 in yeastSWEETs have been shown to mediate the sugar transport in
Arabidopsis thaliana and Oryza sativa as uniporters which do not
require a proton gradient [31,33,51]. To check whether it was
involved in sugar transport, OsSWEET5 was expressed in yeast.
The growth of the mutant strain was restored only on the culture
medium containing galactose but not glucose, fructose, mannose,
or sucrose (Figure 3), suggesting that OsSWEET5 was involved in
galactose transport.
Phenotypes resulting from overexpression of OsSWEET5at seedling stage
To further explore the function of OsSWEET5 in rice,
OsSWEET5-overexpressing plants were generated and single-copy
transgenic plants were confirmed by Southern blot (Figure S4).
Most of the transgenic plants showed a phenotype of growth
retardation. Four homozygous transgenic lines in T2 generation
were further analyzed. The results showed that the plant height
and root length of the overexpression lines were markedly lower
than that of WT plants at seedling stage, indicating a phenotype of
growth retardation (Figure 4A). In addition, the chlorophyll levels
in transgenic lines were significantly lower than those in WT plants
(Figure 4B). Further, Northern blot analysis showed varying
degrees of increased transcript abundance of OsSWEET5 in the
leaves of the transgenic plants (Figure 4C). Since SGR is a
senescence-specific gene in rice and can be used as a molecular
marker for leaf senescence [52,53], the expression of SGR was
examined. As shown in Figure 4D, the expression levels of SGR
were higher in the leaves of OX1 and OX2 than in that of WT
plants. These findings revealed that the overexpression of
OsSWEET5 caused growth retardation and precocious senescence
OsSWEET5 Regulates Growth and Senescence in Rice
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http://www.cbs.dtu.dk/services/TMHMM/http://www.cbs.dtu.dk/services/TMHMM/http://bp.nuap.nagoya-u.ac.jp/sosui/http://bp.nuap.nagoya-u.ac.jp/sosui/
in rice, and the phenotypes were positively correlated with the
expression levels of OsSWEET5. A homozygous positive line
(OX2) with less growth retardation was selected to further explore
the reasons for the abnormal phenotypes.
Abnormal sugar metabolism and transport in OsSWEET5-overexpressing plants
It was shown that OsSWEET5 was involved in galactose
transport in yeast (Figure 3). Therefore, the phenotypes of
OsSWEET5-overexpressing plants may be due to the imbalance
of galactose distribution. To verify this, galactose levels in the
leaves of OX2 and WT at three-leaf stage were analyzed. The
result showed that the galactose level was significantly higher in
OX2 leaves than in WT leaves (Figure 5A). To understand the
cause of the galactose accumulation, the expression levels of the
genes involved in galactose metabolism were examined using
qRT-PCR. As shown in Figure 5B, in the OX2 plants, the
expression levels of b-lactase2, GalM4 and GalK1 were much higherthan those in the WT plants, whereas the expression of GalT was
slightly lower. b-Lactase (encoded by b-lactase2) is involved in thebreakdown of polysaccharide to generate free b-D-Gal, which isconverted to a-D-Gal by galactose mutarotase (encoded by GalM)[54,55]. And then a-D-Gal is phosphorylated by galactokinase(encoded by GalK) and converted to UDP-Gal by a-D-galactose-1-phosphate uridylyltransferase (encoded by GalT) for further
metabolism [55,56]. The qRT-PCR result indicated that the
galactose metabolism was changed, which could have impaired the
galactose distribution.
To investigate whether the levels of other sugars were altered,
sucrose, glucose and fructose levels were also evaluated. Similar to
the level of galactose, the levels of glucose and fructose in the
leaves of OX2 were enhanced to about 2-fold higher than in those
of WT, whereas the level of sucrose was significantly decreased
(Figure 5A). To reveal the reasons for the changes, we further
analyzed the expression of sucrose cleavage genes using qRT-
PCR. As shown in Figure 5B, the transcripts of Inv1, Sus1 and Sus2
were more obviously increased in OX2 than in WT, indicating
that the degradation of sucrose was accelerated in OX2. To check
whether the sugar transport was changed or not, we investigated
the expression levels of the genes involved in sugar transport by
qRT-PCR. As shown in Figure 5C, compared with WT plants,
OX2 displayed dramatically reduced transcripts of OsTMT1,
OsTMT2, OsSUT1 and OsSUT2 (Figure 5C), suggesting that sugar
transport was altered in OX2 compared with in WT plants.
Inhibition of auxin signaling and translocation inOsSWEET5-overexpressing plants
Galactose has long been known to be toxic to plant cell and lead
to growth retardation through the inhibition of auxin signaling
and translocation [18,21,57]. To understand the causes of the
phenotypes in OsSWEET5-overexpressing plants, we evaluated the
IAA levels in the transgenic line (OX2) and WT plants at seedling
Figure 1. Histochemical localization of GUS expression in POsSWEET5::GUS transgenic rice. (A) flag leaf at 40 days after heading; (B) stamen;(C) pistil; (D) hull; (E) stem; (F) root at flowering stage.doi:10.1371/journal.pone.0094210.g001
Figure 2. Subcellular localization of OsSWEET5 in rice cell protoplasts. Rice cell protoplasts were transformed using 35S::OsSWEET5-GFP (A–D) and 35S::GFP (E–G). (B) red autofluorescence signals. (C) and (F) bright field. (D) and (G) merged image. 35S::GFP was transformed as a control. Thebar indicates 20 mm.doi:10.1371/journal.pone.0094210.g002
OsSWEET5 Regulates Growth and Senescence in Rice
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stage. As shown in Figure 6A, the free IAA level was significantly
reduced in the leaves of OX2 compared with in those of WT. The
lower free IAA level may explain why the transgenic plants
exhibited low-auxin phenotypes including dwarfing and the
reduction in shoot and root length (Figure 4A).
To investigate the reasons for the decreased IAA level in
transgenic plants, we further examined the expression levels of
auxin-regulated genes in the leaves of OX2 and WT plants using
qRT-PCR. As shown in Figure 6B, the expression levels of
OsGH3-2 and SAUR39 were markedly increased in OX2
compared with in WT. In addition, the transcripts of OsPIN1,
IAA24 and IAA31 were sharply reduced in OsSWEET5-overex-
pressing plants (Figure 6B). Taken together, these results suggested
that auxin signaling and translocation were inhibited in OX2
plants.
Discussion
OsSWEET5 is involved in galactose transport in riceMany SWEETs have been proven to have sugar transport
ability and function as facilitators that support both the import and
the efflux of sugar into and out of cells [31,33,58]. However,
OsSWEET5 could catalyze the transport of galactose but not that
of glucose, fructose, mannose and sucrose when expressed in yeast
(Figure 3), which is different from other published SWEETs
[9,31,33,36]. This result suggests that OsSWEET5 plays different
roles in rice.
Analysis of the GUS expression patterns in POsSWEET5::GUStransgenic plants revealed that OsSWEET5 was expressed insenescing leaves (Figure 1), which suggests the possibility that
OsSWEET5 participates in the re-import of galactose into the cell
for further metabolism. In addition, many plasma membrane-
localized monosaccharide transporters were expressed in the sink
tissues, suggesting that these transporters might participate in
phloem unloading and supply energy and monosaccharide to sink
tissues [58]. OsSWEET5 was also expressed in the stem, root andfloral organs, which indicates that OsSWEET5 may function in
the mobilization of galactose reserves into these tissues.
Overexpression of OsSWEET5 causes galactoseaccumulation and disordered sugar distribution
The cell wall is a storage reserve of carbon for the plant body
and responds to abnormal circumstances, which leads to the
modification of cell wall polysaccharides, and the resulted sugars
are imported into the cell for further metabolism [28,59]. The
expression of b-lactase2 was up-regulated in the leaves of OX2(Figure 5B). Since b-lactase is involved in the breakdown ofpolysaccharide to generate free b-D-Gal, the up-regulatedexpression of b-lactase2 indicated that cell wall reconstructionwas accelerated in transgenic plants to release galactose. In
addition, the expression levels of three key genes of Leloir salvage
pathway (GalM, GalK and GalT) were significantly altered in OX2,and b-lactase2 and GalM4 showed higher degree of increase inexpression level compared with GalK1 and GalT, leading to theaccumulation of galactose (Figure 5A, B).
Figure 3. OsSWEET5 had sugar transporter activity involved in galactose. Growth complementation of the yeast mutant strain EBY.VW4000was restored by OsSWEET5 on the culture medium containing galactose. N, negative control; P, positive control; OsSWEET5, p413-pHXT7-OsSWEET5.doi:10.1371/journal.pone.0094210.g003
Figure 4. Phenotype and physiological characterization of OsSWEET5-overexpressing transgenic plants. (A) Photographs of WT andOsSWEET5-overexpressing lines (T2) at 15 days after germination. The bar indicates 10 cm. (B) Measurement of chlorophyll content in OsSWEET5-overexpressing lines and WT plants. The samples were from the second leaves in (A). The results shown are the means of three independentmeasurements. Significant differences are calculated by t-test and shown by asterisks. *, P,0.05 or **, P,0.01. FW, Fresh weight. (C) Northern blotanalysis of OsSWEET5-overexpressing lines. RNA was extracted from the second leaves in (A). (D) RT-PCR analysis of SGR in OsSWEET5-overexpressinglines (OX1 and OX2) and WT plants. The first-strand cDNAs were prepared using RNAs extracted from the second leaves of OX1, OX2 and WT plants atthree-leaf stage.doi:10.1371/journal.pone.0094210.g004
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Sugar distribution in the whole plant plays an important role in
the carbohydrate transport for sink tissues, which is important for
the plant growth, and disordered sugar distribution will lead to
abnormal growth in plants [8,60]. Our study showed that
compared with the leaves of the WT plants, OX2 leaves displayed
sharply increased level of monosaccharides (Figure 5A) and
significantly lower expression levels of OsTMT1 and OsTMT2
(Figure 5C). This result suggested that the transport of monosac-
charides from the cytosol to the vacuole lumen was not
accelerated. Moreover, the level of sucrose was significantly
decreased (Figure 5A). The decreased level of sucrose may cause a
lower level of sucrose transport from the source to the sink in OX2
plants. The most obvious effect was the reduced expression of
OsSUT1 and OsSUT2 (Figure 5C), suggesting that the lower level
of sucrose transport from source to sink in OX2 plants reduced the
metabolic flux and thereby led to the phenotype of growth
retardation (Figure 4A). The growth retardation phenotype of the
transgenic plants was similar to the phenotypes of atsweet11ats-
weet12 and ossut2 [8,33]. These results indicated that the carbon
partitioning at the whole plant level was disordered, which led to
the abnormal growth of the transgenic plants. In addition, sugar
has hormone-like functions in regulating many genes and
modulates plant growth and development similarly to phytohor-
mones [10], and different sugar signals are generated by
photosynthesis and carbon metabolism in source and sink tissues
in plants [61]. Hence, all or part of phenotypes of the OsSWEET5-
overexpressing transgenic plants might be ascribed to the
disordered sugar distribution.
Figure 5. Sugar metabolism and transport were disordered inOsSWEET5-overexpressing plants. (A) Sugar levels in leaves of OX2and WT at three-leaf stage at the end of the light periods. Gal,galactose; Suc, sucrose; Glc, glucose; Fru, fructose. Statistical signifi-cance is indicated by * (P,0.05) and ** (P,0.01) (t-test, n = 3). FW, Freshweight. (B) Expression analysis of key genes involved in sugarmetabolism in OX2 and WT plants. The first-strand cDNAs wereprepared using RNAs extracted from the second leaves of OX2 and WTplants at three-leaf stage. c qRT-PCR analysis of genes involved in sugartransport in OX2 and WT plants. The first-strand cDNAs were preparedusing RNAs extracted from the second leaves of OX2 and WT plants atthree-leaf stage.doi:10.1371/journal.pone.0094210.g005
Figure 6. Auxin signaling and translocation were inhibited inOsSWEET5-overexpressing line (OX2) compared to WT plants.(A) Quantification of free IAA contents in the second leaves of OX2 andWT plants at three-leaf stage. Values are means 6SD (n = 3). Statisticalsignificance is indicated by * (P,0.05, t-test). (B) Expression levels ofauxin-regulated genes in the leaves of OX2 and WT plants using qRT-PCR. The first-strand cDNAs were prepared using RNAs extracted fromthe second leaves of OX2 and WT plants at three-leaf stage.doi:10.1371/journal.pone.0094210.g006
OsSWEET5 Regulates Growth and Senescence in Rice
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Galactose accumulation and sugar distribution result inthe inhibition of auxin signaling and translocation
It has been reported that galactose is an important component
of the xyloglucans in the primary cell wall [62]. Nevertheless, free
galactose has severe inhibitory effects on certain aspects of plant
growth and development even at very low concentrations
[21,57,63], and its inhibitory effect on auxin-induced growth
could be explained by the inhibition of IAA transport [57]. In
addition, excessive galactose in plants can inhibit the auxin
biosynthesis and translocation directly or indirectly, and even
induce leaf darkening or chlorosis and growth arrest [18]. In this
study, no significant difference was observed in the expression
levels of the genes involved in ethylene biosynthesis between the
OX2 and WT plants (data not shown), which indicates that the
phenotypes of OX2 plants were not caused by the accumulation of
ethylene. Nevertheless, the free IAA level was significantly
decreased in the OX2 plants with reduced transcripts of auxin
signaling and translocation genes including OsPIN1, IAA24 andIAA31 (Figure 6). In addition, the expression levels of OsGH3-2and SAUR39 were markedly increased in OX2 compared with inWT (Figure 6B). It has been reported that OsGH3-2 encodes anIAA-amido synthetase and inactivates IAA by conjugating it to
amino acids to suppress auxin signaling in rice, and the activation
of OsGH3-2 promoted the formation of IAA-amido, resulting in adecrease in the free IAA level in the OsGH3-2 overexpressing lines[46,64]. SAUR39 acts as a negative regulator of auxin synthesis
and transport in rice, and SAUR39-overexpressing plants displayedreduced growth rate and earlier senescence progression compared
with WT plants [14]. These results suggest that auxin signaling
and translocation have been inhibited to retard the growth of the
OsSWEET5-overexpressing plants.
Sugars can regulate many important processes which are also
controlled by hormones including auxin during plant growth and
development [65]. The crosstalk of sugar and auxin was also
observed in the OX2 plants in our work. In this study, the
expression levels of Inv1 and Sus were increased in OX2 comparedwith in WT (Figure 5B), suggesting that the hydrolysis of Inv- and
Sus-mediated sucrose degradation was accelerated. On one hand,
the ratio of hexose to sucrose is an important factor in the
regulation of IAA biosynthesis [12]. Hence, the lower IAA level in
OX2 plants may be due to the higher ratio of hexose to sucrose
(Figure 5A, 6A). On the other hand, hexoses released from Inv- or
Sus-mediated sucrose degradation can modulate a variety of
developmental processes through interacting with diverse path-
ways including hormonal regulation and PCD pathways [66],
which correlates with the lower IAA and chlorophyll levels in OX2
plants (Figure 4B, 6A). In addition, the phenotypes in OX2 plants
in our work were in conformity with the findings reported
previously. As has been reported, an inverse relation between a
lower auxin level and higher sugar content has been observed in
Arabidopsis [10]. A lower auxin level would lead to an increased
sugar level, which would repress the expression of photosynthetic
genes and chlorophyll production, and eventually cause the
growth retardation phenotypes including leaf senescence and
smaller shoot and root [14,15].
Knockout of OsSWEET5 causes no obvious phenotypesSince OsSWEET5-overexpressing plants displayed growth
retardation phenotype, we generated knockout lines using
amiRNA method (Methods S2) to further explore the function
of OsSWEET5 in rice. The expression of OsSWEET5 wassignificantly suppressed in amiRNA-OsSWEET5 transgenic lines(Figure S5A). However, no obvious phenotype was observed in the
amiRNA-OsSWEET5 transgenic lines (Figure S5B, C). The results
of qRT-PCR showed that the transcript levels of genes involved in
galactose metabolism, sucrose metabolism and transport were not
changed in amiRNA-OsSWEET5 transgenic lines with the excep-
tion of Sus1 (Figure S5D, E). One possible explanation for this is
that there might be an abundance of galactose transporters in rice.
Indeed, the expression of AtSWEET13 was significantly induced in
the atsweet11atsweet12 double mutant compared with in the WT
plants [33], suggesting that SWEET genes are functionally
redundant [67]. Hence, there might be other sugar transporters
which can complement the galactose transport in the amiRNA-
OsSWEET5 plants.
Conclusions
In summary, we identified a galactose transporter gene named
OsSWEET5 in rice. The OsSWEET5-overexpressing plants
showed the phenotypes of growth retardation, precocious senes-
cing leaves and changed sugar content with a reduced auxin level
at seedling stage. These phenotypes might be attributed to the
sugar and auxin crosstalk. The results of the present study will
facilitate a better understanding on the roles of OsSWEET5 as a
galactose transporter in the growth regulation of rice. Further
studies on the silencing of double/multiple genes might help to
elucidate the roles of OsSWEET5 and thus to delineate how the
crosstalk between sugar and auxin modulates rice growth and
development. In addition, optimizing the expression of sugar
transport genes is advantageous for carbohydrates transport and
reserve, which may greatly facilitate the genetic improvement of
yield in rice.
Supporting Information
Figure S1 Sequence alignment of MtN3 family proteinsusing the Clustal_X program. The predicted MtN3 domainswere denoted by underline. The accession numbers of these
proteins are as follows: OsSWEET5 (NP_001056475), Sorghum
bicolor (XP_002441609), Brachypodium distachyon (XP_003576074),
OsSWEET7c/xa25 (Q2QWX8), Zea mays (NP_001149011), Vitis
vinifera (XP_002283068), Solanum lycopersicum (CAE47557), Arabi-
dopsis thaliana (XP_002877087), Glycine max (XP_003553885),
Ricinus communis (XP_002518862), Populus trichocarpa
(XP_002304566), Medicago truncatula (XP_003601464), Os8N3/
xa13 (NP_001062354), OsSWEET14/Os11N3 (NP_001067955).
(TIF)
Figure S2 Expression pattern of OsSWEET5. qRT-PCRanalysis of OsSWEET5 transcript levels in root at seedling with 2
tillers (R1), leaf at secondary branch primordium stage (L1), 4–
5 cm young panicle (P1), flag leaf at 5 days before heading (L2),
stem at heading stage (S), panicles at heading stage (P2), lemma at
1 day before flowering (Le), rachis at 1 day before flowering (Ra),
stamen at 1 day before flowering (St), pistil at 1 day before
flowering (Pi), lodicule at 1 day before flowering (Lo), root at 1 day
before flowering (R2), endosperm at 14 days after pollination (En),
and flag leaf at 14 days after heading (L3), respectively. Error bars
indicate standard deviation of three independent experiments.
Actin1 was used as a control for normalization.
(TIF)
Figure S3 OsSWEET5 protein is predicted by TMHMMto contain seven transmembrane helices.
(TIF)
Figure S4 Southern blot analysis of the copy number ofOsSWEET5-overexpressing plants. M: l-EcoT14 I digest
OsSWEET5 Regulates Growth and Senescence in Rice
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DNA marker. Line 1 to 21, OsSWEET5-overexpressing transgenicplants. The single copy insert plants were marked with asterisk.
(TIF)
Figure S5 AmiRNA-OsSWEET5 transgenic plants had nosignificant differencecompared with WT plants. (A)Expression level of OsSWEET5 in two transgenic lines and WTexamined by RT-PCR. RNA was extracted from panicles of two
transgenic lines and WT at flowering stage. Actin1 was used as aninternal control. (B) Photograph of two transgenic lines and WT at
tillering stage. (C) Measurement of chlorophyll content in the
second leaves of transgenic plants and WT at tillering stage.
Values are the means 6 SD (n = 3). (D–E) The expression of genesinvolved in sugar metabolism and transport in two transgenic lines
and WT plants using qRT-PCR. The first-strand cDNAs were
prepared using RNAs isolated from the second leaves of two
transgenic lines and WT at tillering stage. Bar represents mean (3
replicates) 6 standard deviation.(TIF)
Methods S1 Southern blot analysis.(DOC)
Methods S2 AmiRNA construction and rice transforma-tion.
(DOC)
Table S1 Primers used in this study.
(XLS)
Table S2 Predicting structures of transmembrane heli-ces in OsSWEET5 using SOSUI.
(XLS)
Acknowledgments
We thank Dr. Eckhard Boles of Johann Wolfgang Goethe-Universität
Frankfurt for providing yeast mutant and plasmids. We also thank Dr.
Zuoxiong Liu for reading the manuscript.
Author Contributions
Conceived and designed the experiments: YL YZ LL. Performed the
experiments: YZ WH MY. Analyzed the data: YZ. Contributed reagents/
materials/analysis tools: XL. Wrote the paper: YZ YL FZ.
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